beta -Adrenoceptor-mediated cell signaling in the neonatal heart and liver: responses to terbutaline

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$beta$ -Adrenoceptor-mediated cell signaling in the neonatal heart and liver: responses to terbutaline

J. T. Auman, F. J. Seidler, C. A. Tate, and T. A. Slotkin

Department of Pharmacology and Cancer Biology, Duke University Medical Center, Durham, North Carolina 27710

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Terbutaline, a $beta$ ₂-adrenoceptor ( $beta$ ₂-AR) agonist, is a widely used tocolytic that also crosses the placenta to stimulate fetal $beta$ -ARs. The current study examines the effects of terbutaline administeredto neonatal rats. Terbutaline (10 mg/kg sc) given on postnatalday (PN) 2-5 or PN 11-14 elicited significant downregulation ofboth cardiac and hepatic $beta$ -ARs, with a much greater effect inthe liver. Despite the reduction in cardiac $beta$ -ARs, receptor desensitizationwas absent as evidenced by the maintained ability of isoproterenolto stimulate adenylyl cyclase (AC) in membrane preparations. Theunderlying mechanism was dissected by using stimulants that operateat different points in the AC signaling pathway, NaF, forskolin,and Mn²⁺. When administered in the early neonatal period, terbutalinefailed to evoke any changes in cardiac AC activity; however, treatmenton PN 11-14 evoked heterologous sensitization downstream fromthe receptor, evidenced by increases in the response to NaF andforskolin. In the liver, neonatal terbutaline administration eliciteda small ( $approx$ 10%) decrease in the AC response to isoproterenol, aneffect much smaller than the downregulation of $beta$ -ARs (>40%). Inthis tissue, desensitization was again offset by heterologoussensitization of AC signaling. These results indicate that, inthe developing organism, $beta$ -AR-mediated cell signaling responsesare maintained in the face of receptor downregulation throughheterologous induction of downstream signaling elements. Theseunique responses serve to sustain $beta$ -AR signaling in the perinatalperiod.

adenylyl cyclase; liver; $beta$ -adrenoceptor; preterm labor; adenosine 3',5'-cyclic monophosphate; terbutaline; development; tocolysis; heart

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

$beta$ ₂-ADRENOCEPTOR ( $beta$ ₂-AR) agonists, such as terbutaline, are widely used to prevent preterm delivery, a leading cause of infantmorbidity and mortality in the United States (3). In additionto blocking uterine contractions, terbutaline penetrates the placentato stimulate fetal $beta$ -ARs (2, 16). To a large extent, theseeffects are likely to be beneficial if preterm delivery occurs,as catecholaminergic stimulation promotes cardiovascular, respiratory,and metabolic adaptations that are necessary for perinatal survival(9). However, neonates from mothers receiving tocolytic therapyalso exhibit adverse effects, including tachycardia, alterationsin glucose metabolism (4), and elevated incidence of cardiacanomalies (12, 17).

Both the positive and negative effects of prenatal terbutaline exposure are likely to reflect the result of prolonged, excessive $beta$ -AR stimulation. In adult tissues, $beta$ -AR responses are limitedby receptor downregulation and receptor uncoupling from cell signaling,best exemplified by desensitization of the adenylyl cyclase (AC)signaling cascade (25). However, immature tissues appear tobe resistant to desensitization (23, 24, 27, 30), andwe recently found that $beta$ -AR/AC responses are maintained in theface of repeated terbutaline administration in fetal rats (1).The current study extends this work into the neonatal period,a developmental stage in rats that corresponds more closely tothe status of sympathetic innervation of peripheral tissues inthe third trimester human fetus (9), the period in which terbutalinewould most likely be used. We assessed the ability of terbutalineto induce receptor downregulation and desensitization of $beta$ -ARsignaling after treatment on postnatal (PN) days 2-5, before theonset of sympathetic function, and on PN 11-14, the period inwhich innervation shows its most rapid development (19). Wecompared effects in the heart and liver, tissues that differ inthe predominant $beta$ -AR subtype ( $beta$ ₁ in the heart, $beta$ ₂ in the liver).These tissues also represent major targets for the catecholaminesin the perinatal transition, mediating essential cardiovascularand metabolic adjustments (9). In addition to assessment of $beta$ -ARs and $beta$ -AR-mediated responses, we determined AC responsesto stimulants that bypass the receptors to act on G proteins oron AC itself, so as to dissect the heterologous, downstream mechanismsunderlying resistance to $beta$ -AR desensitization (1, 24).

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Animal treatments. Studies were carried out in accordance with the declaration of Helsinki and with the Guide for the Care and Use of LaboratoryAnimals as adopted and promulgated by the National Institutesof Health. Timed pregnant female Sprague-Dawley rats (Zivic-MillerLaboratories, Allison Park, PA) were shipped by climate-controlledtruck (transit time, 12 h) and housed with free access to foodand water. After birth, pups were randomized and redistributedto the nursing dams with litter sizes maintained at 10 pups; damswere periodically reassigned to different litters to distributeany maternal differences equally. Within each litter, equal numbersof males and females were assigned to each treatment group. Pupswere given daily subcutaneous injections of 10 mg/kg of terbutalinehemisulfate or an equivalent volume (1 ml/kg) of isotonic salinevehicle on PN 2-5 or on PN 11-14. This regimen has been shownpreviously to elicit robust $beta$ ₂-AR downregulation in the adultand to evoke cardiac activation and enhancement of lung surfactantsynthesis in the fetus (1, 8, 16). Twenty-four hours afterthe final injection, hearts, and livers were dissected, frozenin liquid nitrogen, and stored at $-$ 45°C until assayed. Determinationson PN 6 required two hearts for eachassay.

Membrane preparation. Tissues were thawed and homogenized (Polytron, Brinkmann Instruments, Westbury, NY) in 39 volumes of ice-cold buffer containing145 mM NaCl, 2 mM MgCl₂, and 20 mM Tris (pH 7.5) strained throughseveral layers of cheesecloth when necessary to remove connectivetissue and sedimented at 40,000 g for 15 min. The pellets werewashed twice by resuspension (Polytron) in homogenization bufferfollowed by resedimentation and were then dispersed with a homogenizer(smooth glass fitted with a Teflon pestle) to achieve a finalprotein concentration (determined with Folin reagent) of 0.5-1mg/ml in a buffer consisting of 250 mM sucrose, 1 mM EGTA, and10 mM Tris (pH 7.4).

$beta$ -AR binding. Receptor binding capabilities were assessed by methods described in earlier publications (7, 15). The overall strategywas to examine binding of [¹²⁵I]iodopindolol at a single, subsaturating ligand concentration(67 pM) in preparations from each animal; changes can therebybe detected regardless of whether they result from alterationsin receptor dissociation constant or maximal binding (B_max). Thisapproach was necessitated by the requirement to measure bindingin hundreds of membrane preparations in the study; earlier workindicates that receptor downregulation elicited by terbutaline,administered to either fetal or adult rats, reflects a decreasein B_max (1). Binding was determined in samples containing $<=$ 200µg of membrane protein in 250 µl of 145 mM NaCl, 2 mM MgCl₂, 1mM sodium ascorbate, 20 mM Tris (pH 7.5); samples were incubatedfor 20 min at ambient temperature, and labeled membranes weretrapped by vacuum filtration onto glass fiber filters. Nonspecificbinding was determined by displacement with 100 µM D,L-isoproterenoland ranged from 7 to 25%, depending on age andtissue.

AC activity. Aliquots of membrane preparation containing 25-50 µg protein were incubated for 30 min at 30°C with final concentrations of100 mM Tris · HCl (pH 7.4), 10 mM theophylline, 1 mM ATP, 2 mMMgCl₂, 1 mg/ml bovine serum albumin, and a creatine phosphokinase-ATP-regeneratingsystem consisting of 10 mM sodium phosphocreatine and 8 IU/mlphosphocreatine kinase, with or without 10 µM GTP in a total volumeof 250 µl. The enzymatic reaction was stopped by placing the samplesin a 90-100°C water bath for 5 min, followed by sedimentationat 3,000 g for 15 min, and the supernatant solution was assayedfor cAMP using radioimmunoassay kits. Preliminary experimentsshowed that the enzymatic reaction was linear well beyond theassay period and was linear with membrane protein concentration;concentrations of cofactors were optimal and, in particular, theaddition of higher concentrations of GTP produced no further augmentationofactivity.

We assessed the contributions of G protein-linked processes to AC in several ways. First, we contrasted basal AC activityin the presence or absence of GTP. Second, we determined $beta$ -adrenergicstimulation of activity via G_s with 100 µM L-isoproterenol inthe presence of GTP. Third, to determine the net G protein-linkedresponse of AC activity with maximal activation of all G proteins,samples were prepared containing 10 mM NaF in addition to GTP(28). Fourth, we determined the response of AC to 100 µM forskolinor 10 mM MnCl₂ in the presence of GTP. Forskolin requires associationof G proteins with AC for maximal effect (18), whereas Mn²⁺ activates AC by replacing magnesium at the active site (13)and shows decremental effects when G proteins are associated withthe enzyme (28). The preference for one stimulant over the otheralso reflects shifts in the subtype of AC being expressed (28).Finally, to determine whether effects on $beta$ -adrenoceptor signalingrepresented heterologous changes influencing multiple receptorinputs, we assessed the response to clonidine, an $alpha$ ₂-receptoragonist, using a concentration (500 µM) previously found to inhibitAC maximally (20). The effect of clonidine was assessed in liversamples in which AC was first stimulated by isoproterenol or forskolin(20).

Data analysis. Data are presented as means and SE. For convenience, some data are presented as the percent change from control values, butstatistical differences were always established using the originaldata. To establish treatment differences in receptor binding orAC activity, a global ANOVA (data log transformed whenever variancewas heterogeneous) was first conducted across the in vivo treatmentgroups, age, sex, tissue, and for AC, all in vitro conditionsunder which AC was determined; the in vitro stimulant conditionswere repeated measures, because each membrane preparation wasused for the multiple types of AC determinations. As justifiedby significant interactions of treatment × age and treatment ×tissue (see RESULTS), data were then subdivided to permit testingof individual treatments and AC measures that differed from controlvalues; these were conducted by lower-order ANOVAs, followed,where appropriate, by Fisher's protected least-significant differenceto identify specific ages at which the terbutaline group differedfrom the corresponding control. However, in situations where therewas no interaction of treatment × age, only main treatment effectsare reported without conducting separate tests for each age. Testsof drug effects on body and tissue weights and on tissue membraneprotein concentration were evaluated by similar procedures. Forall tests, significance for main treatment effects was assumedat P < 0.05; however, for interactions at P < 0.1, we also examinedwhether lower-order main effects were detectable after subdivisionof the interactive variables (22).

Materials. cAMP radioimmunoassay kits were purchased from Amersham (Chicago, IL) and [¹²⁵I]iodopindolol (specific activity 2,200 Ci/mmol) was obtainedfrom New England Nuclear (Boston, MA). All other chemicals wereobtained from Sigma Chemical (St. Louis,MO).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Development of control rats. Cardiac $beta$ -AR binding increased between PN 6 and PN 15, paralleled by a large augmentation ofthe AC response to $beta$ -AR stimulation by isoproterenol (Table 1).There was no change in basal AC activity, but the coupling ofG proteins to AC showed a substantial rise over this period, evidencedby a greater response to the addition of GTP (15% increase onPN 6, 180% increase on PN 15). Although the response to maximalactivation of all G proteins with NaF also increased over thisperiod, the degree of increase was smaller than that for GTP alone(age × stimulant, P < 0.0001). At both age points, forskolin producedmassive stimulation of AC, much greater than the response to Mn²⁺ (main effect of stimulant, P < 0.0001); the preference for forskolinover Mn²⁺ increased significantly between PN 6 and PN 15 (age × stimulant,P < 0.0001).

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Table 1. $beta$ -Adrenoceptor binding and AC activities in control tissues

In contrast to the heart, $beta$ -AR binding in the liver decreased by one-third between PN 6 and PN 15, consistent with earlierreports (7, 15). Indexes of AC activity also showed an overalldecrease during this period (main effect of age, P < 0.0001).The proportional stimulation evoked by addition of GTP remainedsimilar ( $approx$ double basal activity), as did the response to isoproterenol( $approx$ double the activity compared with +GTP) or NaF ( $approx$ 7 times +GTP),so that all of them decreased in parallel. Although the liver,like the heart, displayed a preferential stimulation by forskolincompared with Mn²⁺ (main effect of stimulant, P < 0.0001), the preference ratiowas substantially smaller than seen in the heart (tissue × stimulant,P < 0.0001) and did not show a significant change with age (stimulant× age, notsignificant).

General effects of terbutaline. Neonatal terbutaline treatment on PN 2-5 or PN 11-14 did not cause any mortality and failed to alter body weight, heart weight,or liver weight nor did it affect the concentration of membraneproteins (Table 2). Accordingly, results for $beta$ -ARs and AC arecompared on the basis of binding or activity per milligram ofmembrane protein, so as to correct for any sample-to-sample variabilityin the recovery of membranes. Given the lack of significant effecton the membrane protein concentration, differences in $beta$ -ARs andAC were also detectable when values were determined per gram oftissue.

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Table 2. Effects of neonatal terbutaline on body and tissue weights and on membrane protein concentration

Global statistical analysis of the effects of terbutaline across both treatment regimens and both tissues indicated a significantoverall reduction of $beta$ -AR binding in the terbutaline group (maineffect of treatment, P < 0.0001) with distinct differences betweenheart and liver (treatment × tissue, P < 0.0001) but no age specificity(not significant for treatment × age or treatment × tissue × age).In contrast, effects on AC activity were both tissue and age specificand differed among the various AC measurements: P < 0.01 for maineffect of treatment, P < 0.09 for treatment × age × tissue, P< 0.0001 for treatment × AC measure, P < 0.0001 for treatment× tissue × AC measure, P < 0.06 for treatment × age × tissue ×AC measure. Given the significant differences in the effects ofterbutaline on heart vs. liver, the results are presented separatelyfor eachtissue.

Effects of terbutaline on the heart. When neonatal rats were given terbutaline on PN 2-5 or PN 11-14, there was a 15-20% decrement in cardiac $beta$ -AR binding, comparableto what is seen in fetal or adult heart after terbutaline treatment(1; Fig. 1). Despite the significant $beta$ -AR downregulation, neithertreatment regimen elicited desensitization of $beta$ -AR-mediated ACactivity, as assessed by the response to isoproterenol, the responseto isoproterenol relative to GTP alone (isoproterenol/+GTP ratio),or the response to isoproterenol relative to maximal G proteinstimulation with NaF (isoproterenol/NaF ratio). For other AC stimulants,however, there were distinct disparities in the effects of thetwo regimens. On PN 6, 24 h after the last injection of the earlytreatment regimen, there were no changes in any of the componentsof AC activity. However, with later terbutaline treatment (PN11-14) there was significant induction of basal AC activity andof the responses to NaF or forskolin. The induction was selectivefor forskolin compared with the other direct AC stimulant, Mn²⁺, as evidenced by a significant decrease in the Mn²⁺/forskolin ratio.

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Fig. 1. Effects of neonatal terbutaline treatment [10 mg/kg sc daily on postnatal day (PN) 2-5 or PN 11-14] on cardiac $beta$ -adrenergic receptor ( $beta$ -AR) binding and adenylyl cyclase (AC) activity. Data represent means and SE obtained from 8-16 determinations in each treatment group at each age, presented as the percentage change from control values (Table 1). ANOVA across all AC measures appears at the top of A, with subdivision by measure at the bottom of A and of B. *Individual values for which the terbutaline group differs from the corresponding control, evaluated only where ANOVA indicated a significant interaction of treatment × age; otherwise, only main effects are reported. Rx, treatment; Iso, isoproterenol.

Effects of terbutaline on the liver. Neonatal terbutaline had a much greater effect on hepatic $beta$ -AR binding than on cardiac $beta$ -ARs (treatment × tissue, P < 0.0001;Fig. 2). Values were decreased by 40% regardless of whether treatmentoccurred in the early neonatal period (PN 2-5) or in the secondpostnatal week (PN 11-14). Despite the marked decline in $beta$ -ARs,the ability of isoproterenol to stimulate AC activity was onlyslightly reduced (10-15%), an effect clearly distinguishable fromthe robust receptor downregulation (treatment × measure, P < 0.0001).Examination of the effects on the AC response to stimulants downstreamfrom the $beta$ -AR indicated that heterologous sensitization of thesignaling pathway offset the effects of homologous desensitizationof receptor-mediated signaling. On PN 6, the AC responses to NaF,forskolin, or Mn²⁺ all were elevated (main effect of treatment, P < 0.0001). Theactivity ratios confirmed that the increases in G protein-mediatedand total AC catalytic activity were able to offset homologousdesensitization: there were significant decreases in the isoproterenol/+GTPand isoproterenol/NaF activity ratios (main effect of treatment,P < 0.0001), with a greater effect on the latter ratio (treatment× measure, P < 0.0001), as would be expected from differentialeffects on the $beta$ -AR signaling component. With treatment on PN11-14, the same directional changes were seen except for smallernet effects on the responses to forskolin and Mn²⁺ (treatment × age, P < 0.04).

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Fig. 2. Effects of neonatal terbutaline treatment (10 mg/kg sc daily on PN 2-5 or PN 11-14) on hepatic $beta$ -AR binding and AC activity. Data represent means and SEs obtained from 8 determinations in each treatment group at each age, presented as the percentage change from control values (Table 1). ANOVA across all AC measures appears at the top of A, with subdivision by measure at the bottom of A and of B. *Individual values for which the terbutaline group differs from the corresponding control, evaluated only where ANOVA indicated a significant interaction of treatment × age; otherwise, only main effects are reported.

Because our results suggested that neonatal terbutaline treatment elicits heterologous effects involving G proteins, we examinedthe effects of clonidine, an $alpha$ ₂-AR agonist that normally inhibitsAC through its coupling to G_i. Samples were prepared in the absenceor presence of a maximally effective concentration (500 µM) ofclonidine (20), superimposed on the stimulant effects of isoproterenolor forskolin (Fig. 3). In control rats, clonidine failed to inhibitisoproterenol-mediated AC at either age and instead potentiatedthe stimulant effects (main effect of clonidine, P < 0.0003);in vivo pretreatment with terbutaline did not alter this pattern.When forskolin was used as a stimulant, however, clonidine hadlittle effect on the AC response in controls on PN 6, switchingto a pronounced enhancement of activity on PN 15 (P < 0.005 formain effect of clonidine, P < 0.0007 for clonidine × age). Pretreatmentof neonates with terbutaline promoted the inhibitory actions ofclonidine (treatment × clonidine, P < 0.03), eliciting an outrightinhibitory effect on the forskolin response on PN 6 (P < 0.02)and reducing the stimulatory effect of forskolin on PN 15 (P <0.05).

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Fig. 3. Effects of neonatal terbutaline treatment (10 mg/kg sc daily on PN 2-5 or PN 11-14) on hepatic AC responses to clonidine (500 µM), measured in the presence of isoproterenol (A) or forskolin (B). Data represent means and SE obtained from 8 determinations in each treatment group at each age, presented as the percent change from values obtained without addition of clonidine. ANOVA across all measures appears at the top of A and of B; subdivision into separate ages was not carried out because of the absence of interactions of treatment × age.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Signaling mediated by the $beta$ -AR/AC pathway undergoes major changes in the neonatal period. In the fetus or in the adult, thecardiac AC response to isoproterenol is much smaller than thatseen with global activation of G proteins by NaF (1), whereasin the current study, we found that the two stimulants were equallyeffective in the neonate. Accordingly, the relative efficiencyof $beta$ -AR coupling to AC peaks in this period. In contrast, hepaticAC responses to $beta$ -AR stimulation are highest in the fetus (1)and decline sequentially through the neonatal period into adulthood,paralleling the ontogenetic decline in the expression of $beta$ -ARs(7, 15). The two tissues also differ substantially in theirdevelopmental patterns for catalytic properties of AC (1):throughout development, the heart displays a preferential responseto forskolin vs. Mn²⁺, just as seen here in the neonate, whereas in the liver, Mn²⁺ is more effective than forskolin in the fetus, less effectivein the neonate, and equally effective in the adult. Accordingly,the effects of neonatal terbutaline treatment can be expectedto differ in the two tissues not only because of disparate proportionsof $beta$ ₁- and $beta$ ₂-subtypes but also because of inherent discrepanciesin receptor coupling and in the ontogenetic patterns of G proteinsand ACitself.

In mature cells, prolonged or excessive stimulation of $beta$ -ARs elicits receptor downregulation as a key component of desensitization.However, previous reports indicate that $beta$ -ARs in the neonate areresistant to the downregulation elicited by administration ofisoproterenol, a mixed $beta$ ₁/ $beta$ ₂-agonist (10, 24). In an earlierstudy (1), we found that in the fetus, terbutaline, a $beta$ ₂-selectivedrug, did evoke a small degree of cardiac $beta$ -AR downregulationand a much more robust decrease of hepatic $beta$ -ARs. The currentresults resolve the apparent discrepancy between the downregulationcaused by fetal terbutaline and lack of downregulation seen withisoproterenol in the neonate: terbutaline administered to neonatalrats evoked cardiac and hepatic $beta$ -AR downregulation similar inmagnitude (15 and 40%, respectively) to that seen in the fetusor the adult (1); the relatively greater effect in the liveris expected, given the higher proportion of hepatic $beta$ ₂-ARs (1).Obviously, immature cells contain the machinery necessary to elicitreceptor downregulation, yet are resistant to doing so when isoproterenolis administered instead of terbutaline. There are two possibleexplanations. First, terbutaline and isoproterenol differ in theirpharmacokinetics, with terbutaline providing a much more prolongedeffect. Accordingly, immature cells may be resistant to, albeitnot absolutely incapable of, $beta$ -AR downregulation, requiring muchmore prolonged stimulation to elicit the effect; thus there maybe a relative (but not absolute) deficiency in components necessaryfor downregulation. Alternatively, specificity toward $beta$ ₁- vs. $beta$ ₂-subtypes may elicit different trophic actions on cardiac celldevelopment that offset receptor downregulation, producing anactive response that prevents the loss of receptors from the cellsurface; if this interpretation is correct, it would imply a specificrole for $beta$ ₁-ARs in resistance todownregulation.

Regardless of the presence or absence of $beta$ -AR downregulation, and notwithstanding the marked difference in the degree of downregulationbetween heart and liver, we did not observe desensitization ofAC signaling mediated through $beta$ -ARs, the same result found afterfetal terbutaline exposure (1) or neonatal isoproterenol treatment(30). Again, the issue comes down to two possibilities: is theresomething missing from developing cells that is necessary to receptordesensitization, or are there active processes that are uniqueto developing cells, which offset the effects of desensitization?Our results provide evidence for contributions from both processes.In the heart, terbutaline administered on PN 11-14 produced inductionof AC catalytic activity, evidenced by a significant increasein the enzymatic response to forskolin, with a parallel increasein the response to NaF, which operates through G proteins; wealso detected a shift in catalytic properties of AC, a decreasein the Mn²⁺/forskolin stimulation ratio, indicative of promotion of stimulatoryG protein actions and/or induction of a different AC isoform (28).As $beta$ -ARs also operate through G proteins to stimulate AC, theinduction of responses at these two downstream signaling loci,an active compensatory process that is not seen in mature cells,clearly could offset desensitization at the level of the $beta$ -AR.However, terbutaline treatment on PN 2-5 did not elicit inductionof the responses to forskolin or NaF, but nevertheless the ACresponse to isoproterenol was maintained in the face of receptordownregulation, suggesting that, at this earlier stage, thereis a deficiency in cellular components required fordesensitization.

Of course, a third possibility is simply that the degree of cardiac $beta$ -AR downregulation is simply too small to elicit a correspondingloss of signaling capabilities, especially given the predominanceof the $beta$ ₁-subtype in this tissue. This latter possibility is addressedby our results in the liver, a tissue in which virtually all thereceptors are of the $beta$ ₂-subtype (1) and in which we observedrobust downregulation after neonatal terbutaline administration.Neonates given terbutaline on PN 2-5 showed statistically significantdesensitization of AC responses to $beta$ -AR stimulation, but the lossof the response was far smaller than would be expected from the40% decrease in receptor numbers. Just as in the heart, we observedinduction at the levels of AC (responses to forskolin and Mn²⁺) and G proteins (response to NaF). The heterologous sensitizationof signaling elements downstream from the receptor clearly contributeto the protection from desensitization: when we compared the responseto isoproterenol with that to NaF, we detected homologous desensitization,but the net effect was offset by induction at the level of G proteinsand AC. Notably, however, terbutaline administration on PN 11-14produced the same protection of the $beta$ -AR-mediated AC response,despite much smaller induction of AC. So again, the resistanceof the developing cells to agonist-induced desensitization residesin a combination of active, heterologous processes that offsethomologous receptor downregulation and desensitization, as wellas a deficiency in the processes that mediate desensitization.Future work needs to address what specifically prevents developingcells from efficient desensitization of receptor signals. Prolongedagonist exposure activates G protein receptor kinase 2 (GRK2),which translocates to the membrane to phosphorylate $beta$ -ARs, resultingin recruitment of $beta$ -arrestin to initiate receptor internalization(14). Neonatal hearts contain an excess of GRK2 relative tothe adult (27), yet still do not show $beta$ -AR desensitization,even before induction of AC (27). It is not yet known if $beta$ -ARstimulation effectively recruits GRK2 to the plasma membrane inthe neonatal heart or whether there might be deficiencies in $beta$ -arrestinexpression or function. However, regardless of the actual mechanismresponsible for the deficient ability of neonatal tissues to elicit $beta$ -AR desensitization, the important net result is that $beta$ -AR-mediatedsignaling is maintained regardless of the presence or absenceof reductions in $beta$ -ARsthemselves.

Earlier work with neonatal isoproterenol administration indicated that $beta$ -AR stimulation of immature cardiac cells evokes uniquechanges in the expression and function of stimulatory vs. inhibitoryG proteins, marked by an increase in G_s effect and suppressionof G_i expression (27, 29). In the current study with terbutaline,several of our findings also indicated the targeting of G proteins.If the only effect of terbutaline were to induce total AC activityor a new AC isoform, then basal activity and activity in the presenceof GTP would simply follow suit. Instead, we found differentialeffects on basal AC and activity in the presence of GTP, differencesof these two measures from the effects on the isoproterenol orNaF response, as well as decreases in the Mn²⁺/forskolin activity ratio (28, 29). We therefore examinedthe responses mediated by $alpha$ ₂-ARs, which ordinarily act as a negativemodulators of AC activity through coupling to G_i. We found thatstimulation of neonatal hepatic $alpha$ ₂-ARs potentiated isoproterenol-stimulatedcAMP production, an effect previously observed in the fetal liver(1) and in the pregnant rat myometrium (11). Neonatal terbutalinetreatment did not alter this pattern. Surprisingly, when we usedforskolin as the AC stimulant, we observed a different ontogeneticpattern for $alpha$ ₂-AR-mediated effects: on PN 6, we found a "normal"inhibitory effect of clonidine but on PN 15 we again found a stimulatoryeffect. In this case, neonatal terbutaline administration enhancedthe inhibitory component of the $alpha$ ₂-AR effect, leading to greaterdecreases in AC on PN 6 and smaller increases on PN 15. The resultsindicate a complex relationship of neonatal $beta$ -AR stimulation tothe expression and/or function of $alpha$ -ARs and their coupling toG_i, but the exact nature of this interaction is not clear at thistime. Previously, we found crosstalk of receptor expression between $beta$ -ARs and $alpha$ -ARs in developing heart and liver, effects not seenin mature cells (24). Additionally, $beta$ ₂-ARs couple to both G_sand G_i (26), so that differential effects of terbutaline onthe development of the two G protein classes could produce theresults seen here (29).

The failure of terbutaline to produce effective $beta$ -AR desensitization in the neonatal rat is an important consideration inits use as a tocolytic, because the neonatal rat resembles a thirdtrimester human fetus with respect to sympathetic innervation(9). The effective linkage of the $beta$ -ARs to AC, combined withheterologous sensitization downstream from the receptor, meansthat terbutaline administration will produce profound and prolongedstimulation of fetal target tissues. This is a favorable outcomein that catecholamine actions at $beta$ -ARs are necessary for the cardiovascularand metabolic events that enable the successful transition toextrauterine life (9). At the same time, the fact that $beta$ -ARstimulation elicits changes in target cell differentiation oreven apoptosis (5, 6, 21) means that the failure to desensitizethe receptors in the face of continued stimulation may conferlong-term liabilities. Indeed, abnormalities of neonatal cardiaccontrol and glucose metabolism have been noted after tocolytictherapy (4), along with an increased incidence of cardiac structuralanomalies (12, 17).

In conclusion, neonatal terbutaline exposure produces $beta$ -AR downregulation without reducing the net ability of $beta$ -AR stimulationto elicit an increase in cAMP production. $beta$ -AR signaling is maintainedbecause of deficiencies in the ability of immature cells to uncouplereceptors from response elements, but also because of heterologoussensitization of signaling components downstream from the receptor.Although these processes enable $beta$ -AR function to be maintainedduring the perinatal period, the same processes may promote abnormalitiesin the development of $beta$ -AR target tissues when $beta$ ₂-AR agonistsare used to arrest pretermlabor.

	ACKNOWLEDGEMENTS

This work was supported by National Institute of Child Health and Human Development Grant HD-09713.

	FOOTNOTES

Address for reprint requests and other correspondence: Dr. T. A. Slotkin, Box 3813 DUMC, Dept. of Pharmacology & Cancer Biology,Duke Univ. Med. Ctr., Durham, NC 27710 (E-mail: t.slotkin{at}duke.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 18 June 2001; accepted in final form 23 August 2001.

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